read.bismark: Parsing output from the Bismark alignment suite.

Description Usage Arguments Value File formats Efficient use of read.bismark() Realization backends Parallelization, progress monitoring, and logging Author(s) See Also Examples

View source: R/read.bismark.R

Description

Parsing output from the Bismark alignment suite.

Usage

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read.bismark(files,
             loci = NULL,
             colData = NULL,
             rmZeroCov = FALSE,
             strandCollapse = TRUE,
             BPPARAM = bpparam(),
             BACKEND = NULL,
             dir = tempfile("BSseq"),
             replace = FALSE,
             chunkdim = NULL,
             level = NULL,
             nThread = 1L,
             verbose = getOption("verbose"))

Arguments

files

The path to the files created by running Bismark's methylation extractor, one sample per file. Files ending in .gz or .bz2 will be automatically decompressed to tempfile(). We strongly recommend you use the 'genome wide cytosine report' output files. See section 'File formats' for further details.

loci

NULL (default) or a GenomicRanges instance containing methylation loci (all with width equal to 1). If loci = NULL, then read.bismark() will perform a first pass over the Bismark file to identify candidate loci. If loci is a GenomicRanges instance, then these form the candidate loci. In either case, the candidate loci will be filtered if rmZeroCov = TRUE and collapsed if strandCollapse = TRUE to form the final set of methylation loci that form the rowRanges of the returned BSseq object. See section 'Efficient use of read.bismark()' for further details.

colData

An optional DataFrame describing the samples. Row names, if present, become the column names of the BSseq object. If NULL, then a DataFrame will be created with files used as the row names.

rmZeroCov

A logical(1) indicating whether methylation loci that have zero coverage in all samples be removed. For several reasons, the default rmZeroCov = FALSE is recommended even in cases where you ultimately want to remove such loci. See section 'Efficient use of read.bismark()' for further details.

strandCollapse

A logical(1) indicating whether strand-symmetric methylation loci (i.e. CpGs) should be collapsed across strands. This is only applicable for stranded methylation loci, e.g., loci extracted from 'genome wide cytosine reports' (see section 'File formats' for further details).

BPPARAM

An optional BiocParallelParam instance determining the parallel back-end to be used during evaluation. Currently supported are SerialParam (Unix, Mac, Windows), MulticoreParam (Unix and Mac), SnowParam (Unix, Mac, and Windows, limited to single-machine clusters), and BatchJobsParam (Unix, Mac, Windows, only with the in-memory realization backend). See sections 'Parallelization and progress monitoring' and 'Realization backends' for further details.

BACKEND

NULL or a single string specifying the name of the realization backend. When the backend is set to NULL, the M and Cov assays are realized in memory as ordinary matrices, otherwise these are realized with the given BACKEND. See section 'Realization backends' for further details.

dir

Only applicable if BACKEND == "HDF5Array". The path (as a single string) to the directory where to save the HDF5-based BSseq object. The directory will be created so should not already exist, unless replace is set to TRUE.

replace

Only applicable if BACKEND == "HDF5Array". If directory dir already exists, should it be replaced with a new one? The content of the existing directory will be lost!

chunkdim

Only applicable if BACKEND == "HDF5Array". The dimensions of the chunks to use for writing the data to disk. By default, getHDF5DumpChunkDim() using the dimensions of the returned BSseq object will be used. See ?getHDF5DumpChunkDim for more information.

level

Only applicable if BACKEND == "HDF5Array". The compression level to use for writing the data to disk. By default, getHDF5DumpCompressionLevel() will be used. See ?getHDF5DumpCompressionLevel for more information.

nThread

The number of threads used by fread when reading the files. Be careful when combining a parallel backend specified with BPPARAM with nThread > 1 because each worker will use nThread.

verbose

A logical(1) indicating whether progress messages should be printed (default TRUE).

Value

A BSseq object.

File formats

The format of each file is automatically detected using the internal function bsseq:::.guessBismarkFileType(). Files ending in .gz, .bz2, .xz, or .zip will be automatically decompressed to tempdir().

Supported file formats

Bismark's 'genome wide cytosine report' (https://github.com/FelixKrueger/Bismark/tree/master/Docs#the-genome-wide-cytosine-report-optional-is-tab-delimited-in-the-following-format-1-based-coords) and 'coverage' (https://github.com/FelixKrueger/Bismark/tree/master/Docs#the-coverage-output-looks-like-this-tab-delimited-1-based-genomic-coords) formats are both supported. If setting loci = NULL, then we strongly recommend using the 'genome wide cytosine report' output format because this includes strand information for each locus. The 'coverage' output does not contain strand information and so the strand of the returned BSseq object will be set to * unless stranded loci are supplied.

Unsupported file formats

Neither the 'bedGraph' output format (https://github.com/FelixKrueger/Bismark/tree/master/Docs#the-bedgraph-output-optional-looks-like-this-tab-delimited-0-based-start-1-based-end-coords) nor the 'bismark_methylation_extractor' output format (https://github.com/FelixKrueger/Bismark/tree/master/Docs#the-bismark_methylation_extractor-output-is-in-the-form-tab-delimited-1-based-coords) are supported. The former does not include the required counts of methylated and unmethylated reads hile the is an intermediate file containing read-level, rather than locus-level, data on methylation.

One-based vs. zero-based genomic co-ordinates

The genomic co-ordinates of the Bismark output files may be zero-based or one-based depending on whether the --zero_based argument was used when running Bismark's methylation extractor. Furthermore, the default co-ordinate counting system varies by version of Bismark. bsseq makes no assumptions about the basis of the genomic co-ordinates and it is left to the user to ensure that the appropriate basis is used in the analysis of their data.

Since Bioconductor packages typically use one-based co-ordinates, we strongly recommend that your Bismark files are also one-based.

Efficient use of read.bismark()

We recommend the following to achieve fast and efficient importing of Bismark files:

Each point is discussed below.

Specifying loci

Specifying the set of methylation loci via the loci argument means that read.bismark() does not need to first parse all files to identify the set of candidate loci. Provided that rmZeroCov = FALSE, this means that each file is only read once. This may be a considerable saving when there are a large number of files.

If you are unsure whether the below-described shortcuts apply to your data, leave loci = NULL and let read.bismark() identify the set of candidate loci from files.

You may wish to use the findLoci() function to find all methylation loci of interest in your reference genome (e.g., all CpGs) and then pass the result via the loci argument.

Alternatively, if all files are 'genome wide cytosine reports' for samples aligned to the same reference genome, then all files contain the exact same set of methylation loci. In this case, you may wish to first construct loci using the internal function bsseq:::.readBismarkAsFWGRanges() applied to a single file, e.g., loci = bsseq:::.readBismarkAsFWGRanges(files[1], rmZeroCov, strandCollapse).

Using the 'coverage' Bismark files

It will generally be faster to parse Bismark files in the 'coverage' output format than those in the 'genome wide cytosine report' format This is because the former only includes loci with non-zero coverage and so the file size is often considerably smaller, particularly for shallowly sequenced samples (e.g., those from single-cell bisulfite sequencing).

Leaving rmZeroCov = FALSE

If you set rmZeroCov = TRUE, then read.bismark() must first parse all the files to identify which loci have zero coverage in all samples and then filter these out from the set of candidate loci. This will happen even if you supply loci with a GenomicRanges of candidate loci.

Furthermore, any coverage-based filtering of methylation loci is best left until you have constructed your final BSseq object. In our experience, the final BSseq object is often the product of combining multiple BSseq objects, each constructed with a separate call to read.bismark(). In such cases, it is premature to use rmZeroCov = TRUE when running each read.bismark(); regretably, combining these objects will often then lead to an inefficiently stored BSseq object.

Using a BPPARAM with a moderate number of workers (cores)

Each file can be processed on its own, so you can process in parallel as many files as you have workers. However, if using the HDF5Array backend, then writing to the HDF5 file cannot be performed in parallel and so becomes the bottleneck. Nonetheless, by using a moderate number of workers (2 - 10), we can ensure there is processed data available to write to disk as soon as the current write is completed.

Using BACKEND = "HDF5Array"

By using the HDF5Array realization backend from HDF5Array, we reduce the amount of data that is kept in-memory at any one time. Once each file is parsed, the data are written to the HDF5 file and are no longer needed in-memory. When combined with multiple workers (cores), this means that each file will only need to read and retain in-memory 1 sample's worth of data at a time.

Conversely, if you opt for all data to be in-memory (via BACKEND = NULL), then each worker will pass each file's data back to the main process and memory usage will steadily accumulate to often unreasonable levels.

Using nThread > 1

read.bismark uses data.table::fread to read each file, which supports threaded-parallisation. Depending on the system, increasing nThread can achieve near-linear speed-ups in the number of threads for reading each file. Care needs to be taken when nThread > 1 is used in conjunction with a parallel backend via BPPARAM to ensure the system isn't overloaded. For example, using BPPARAM = MulticoreParam(workers = 10) with nThread = 4 may use up to 40 workers simultaneously.

Realization backends

The read.bismark() function creates a BSseq object with two assays, M and Cov. The choice of realization backend controls whether these assays are stored in-memory as an ordinary matrix or on-disk as a HDF5Array, for example. The choice of realization backend is controlled by the BACKEND argument, which defaults to the current value of DelayedArray::getAutoRealizationBackend().

read.bismark() supports the following realization backends:

Please note that certain combinations of realization backend and parallelization backend are currently not supported. For example, the HDF5Array realization backend is currently only compatible when used with a single-machine parallelization backend (i.e. it is not compatible with a SnowParam that specifies an ad hoc cluster of multiple machines). BSmooth() will issue an error when given such incompatible realization and parallelization backends.

Additional arguments related to the realization backend can be passed via the ... argument. These arguments must be named and are passed to the relevant RealizationSink constructor. For example, the ... argument can be used to specify the path to the HDF5 file to be used by BSmooth(). Please see the examples at the bottom of the page.

Parallelization, progress monitoring, and logging

read.bismark() now uses the BiocParallel package to implement parallelization. This brings some notable improvements:

All parallelization options are controlled via the BPPARAM argument. In general, we recommend that users combine multicore (single-machine) parallelization with an on-disk realization backend (see section, 'Realization backend'). For Unix and Mac users, this means using a MulticoreParam. For Windows users, this means using a single-machine SnowParam. Please consult the BiocParallel documentation to take full advantage of the more advanced features.

A useful feature of BiocParallel are progress bars to monitor the status of long-running jobs, such as BSmooth(). Progress bars are controlled via the progressbar argument in the BiocParallelParam constructor.

BiocParallel also supports extensive and detailed logging facilities. Please consult the BiocParallel documentation to take full advantage these advanced features.

Author(s)

Peter Hickey peter.hickey@gmail.com

See Also

Examples

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  # Run read.bismark() on a single sample to construct a matrix-backed BSseq
  # object.
  infile <- system.file("extdata/test_data.fastq_bismark.bismark.cov.gz",
                        package = "bsseq")
  bsseq <- read.bismark(files = infile,
                        colData = DataFrame(row.names = "test_data"),
                        rmZeroCov = FALSE,
                        strandCollapse = FALSE,
                        verbose = TRUE)
  # This is a matrix-backed BSseq object.
  sapply(assays(bsseq, withDimnames = FALSE), class)
  bsseq

  ## Not run: 
  # Run read.bismark() on a single sample to construct a HDF5Array-backed BSseq
  # object (with data written to 'test_dir')
  test_dir <- tempfile("BSseq")
  bsseq <- read.bismark(files = infile,
                        colData = DataFrame(row.names = "test_data"),
                        rmZeroCov = FALSE,
                        strandCollapse = FALSE,
                        BACKEND = "HDF5Array",
                        dir = test_dir,
                        verbose = TRUE)
  # This is a HDF5Array-backed BSseq object.
  sapply(assays(bsseq, withDimnames = FALSE), class)
  # The 'M' and 'Cov' assays are in the HDF5 file 'assays.h5' (in 'test_dir').
  sapply(assays(bsseq, withDimnames = FALSE), path)
  
## End(Not run)

bsseq documentation built on Nov. 8, 2020, 7:53 p.m.